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在发夹寡核苷酸底物上分析与玉米黑粉菌REC1基因产物相关的DNA水解活性。

DNA hydrolytic activity associated with the Ustilago maydis REC1 gene product analyzed on hairpin oligonucleotide substrates.

作者信息

Naureckiene S, Holloman W K

机构信息

Hearst Microbiology Research Center, Department of Microbiology and Immunology, Cornell University Weill Medical College, New York 10021, USA.

出版信息

Biochemistry. 1999 Oct 26;38(43):14379-86. doi: 10.1021/bi991495b.

Abstract

The REC1 gene of Ustilago maydis functions in the maintenance of genome stability as evidenced by the mutator phenotype resulting from inactivation of the gene. The biochemical function of the Rec1 protein was previously identified as a 3'-5'-directed DNA exonuclease. Here studies on the mechanism of action of Rec1 were performed using radiolabeled oligonucleotide DNAs as substrates, enabling detection of single cleavage events after electrophoresis on DNA sequencing gels. The oligonucleotides that were utilized were designed to be self-annealing so that they formed hairpin structures. This simplified interpretation of the data since each molecule contained only one 3'-terminus. Analysis revealed that digestion proceeded by a distributive mode of action and that degradation of DNA was governed by an interplay between sequence context and conformation. The preferential substrate was DNA with a recessed 3'-end. It was discovered that the enzyme had abasic endonuclease activity, was capable of initiating at an internal nick, and had no preference for mismatched bases either internally or terminally. Endonucleolytic cleavage was 5' to the abasic site.

摘要

玉米黑粉菌的REC1基因在维持基因组稳定性方面发挥作用,该基因失活导致的突变体表型证明了这一点。Rec1蛋白的生化功能先前被鉴定为一种3'-5'定向DNA外切核酸酶。在这里,使用放射性标记的寡核苷酸DNA作为底物对Rec1的作用机制进行了研究,这使得在DNA测序凝胶上进行电泳后能够检测到单个切割事件。所使用的寡核苷酸被设计为自退火的,以便它们形成发夹结构。由于每个分子仅包含一个3'-末端,这简化了数据的解释。分析表明,消化以分布作用模式进行,DNA的降解受序列背景和构象之间相互作用的支配。优先底物是具有凹陷3'-末端的DNA。研究发现,该酶具有无碱基内切核酸酶活性,能够在内部切口处起始,并且对内部或末端的错配碱基没有偏好。内切核酸酶切割发生在无碱基位点的5'端。

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